I have continuous problem with my ChIP - I am using Dynalbeads and following protocol, that has been used in my lab and worked fine. I am working with budding yeast cells, my input values (Input diluted 10x before qPCR reaction) are extremely high - Ct 24 - 29 comparing to +/- antibody - approx. Ct 23/27.
Aftab Alam
You might be taking more number of cells initially. There are lot of calculation methods where IgG is used as control where you do not need the Input Ct value.
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